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Effect of storage and DNA extraction method on 16S rRNA-profiled fecal microbiota in Japanese adults

机译:储存和DNA提取方法对日本成年人16S rRNA谱线粪便菌群的影响

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摘要

The effect of two factors, storage and the bacterial DNA extraction method, that potentially affect the 16S rRNA-based profiling of the microbiota in the feces of Japanese adults, were evaluated. Profiles of the microbiota in feces stored in DESS (DMSO-EDTA-salt solution) for 1, 2 and 3 weeks at room temperature, and for 3 weeks at 4°C were compared with those in fresh feces and feces stored in guanidine thiocyanate solution for 3 weeks at 4°C. None of the storage variables (preservation solution, temperature and duration) considerably affected α- and β-diversity of the fecal microbiota and OTU profiles. Regarding the bacterial DNA extraction methods, four were evaluated; A) silica membrane DNA purification combined with bead-beating bacterial disruption, B) magnetic bead DNA purification combined with bead-beating bacterial disruption, C) manual DNA purification using phenol-chloroform and ethanol precipitation combined with enzymatic bacterial lysis, and D) DNA extraction by a commercially available DNA stool kit. While methods A, B, and C did not markedly affect α- and β-diversity of the fecal microbiota and the OTU profiles, method D noticeably altered both α- and β-diversity. In addition, method D caused significant changes in the abundance of two predominant genera; Bacteroides and Bifidobacterium.
机译:评估了可能影响日本成年人粪便中微生物群基于16S rRNA的谱分析的两个因素(存储和细菌DNA提取方法)的影响。将DESS(DMSO-EDTA-盐溶液)中储存的粪便中的微生物菌群在室温下分别放置1、2和3周,在4°C下放置3周的微生物群图与新鲜粪便和硫氰酸胍溶液中储存的粪便中的微生物群进行了比较在4°C下放置3周。没有任何存储变量(保存溶液,温度和持续时间)显着影响粪便微生物群和OTU分布的α和β多样性。关于细菌DNA的提取方法,评价了4种。 A)硅胶膜DNA纯化与敲除细菌的破坏相结合,B)磁珠DNA纯化与敲击细菌的破坏相结合,C)使用苯酚-氯仿和乙醇沉淀结合酶促细菌裂解的手动DNA纯化,以及D)DNA用市售的DNA粪便试剂盒提取。尽管方法A,B和C对粪便菌群的α和β多样性和OTU分布没有明显影响,但方法D显着改变了α和β多样性。此外,方法D导致两个主要属的丰度发生了显着变化。拟杆菌和双歧杆菌。

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